SELECTIVE REGULATION OF EXPRESSION OF PROTEIN-KINASE-C BETA-ISOENZYMES OCCURS VIA ALTERNATIVE SPLICING

被引:0
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作者
BLOBE, GC
KHAN, WA
HALPERN, AE
OBEID, LM
HANNUN, YA
机构
[1] DUKE UNIV,MED CTR,DEPT MED,DIV HEMATOL ONCOL,BOX 3355,DURHAM,NC 27710
[2] DUKE UNIV,MED CTR,DEPT CELL BIOL,DURHAM,NC 27710
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中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The mechanisms involved in regulating the selective expression of protein kinase C (PKC) isoenzymes are poorly understood. Two human B lymphoblastoid cell lines, IM-9 and BJA-B, exhibited differential expression of the two alternatively spliced products of the PKC beta gene, PKC betaI and betaII. The IM-9 cell line expressed 3-4-fold more PKC betaII protein than the BJA-B cell line, whereas the BJA-B cell line expressed 2-3-fold more PKC betaI protein. This differential expression was found to be regulated at the mRNA level. Comparison of PKC betaI and betaII messages in poly(A)+ mRNA and total cellular RNA revealed that selective polyadenylation was not involved. The messages for PKC betaI and betaII had comparable half-lives in both cell lines, ruling out differential message stability. In addition, similar ratios of PKC betaI and betaII messages in cytosolic and nuclear fractions suggested that differential mRNA transport was not involved. In the IM-9 cell line, the predominance of mature PKC betaII message as well as that of a larger message spliced to PKC betaII provided evidence that the differential expression of PKC betaII was regulated at the level of mRNA splicing. In the BJA-B cell line, equal amounts of mature PKC betaI and betaII message and the absence of the larger message suggested that the splicing of the PKC beta gene product can be regulated to produce altered ratios of PKC betaI and betaII. Implications of these studies on the differential expression of PKC isoenzymes and their roles in biology are discussed.
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页码:10627 / 10635
页数:9
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